JPWO2013137173A1 - Biosensor and manufacturing method thereof - Google Patents

Abstract

Provided is a technique capable of easily producing a biosensor that can be stored for a long period of time by including a hydrophilic polymer that does not have an oxygen atom double bond in each of an enzyme layer and a mediator layer. Since the enzyme layer 106b and the mediator layer 106c are formed together as the reaction layer 106, it is not necessary to form the enzyme layer 106b and the mediator layer 106c separately on the cover layer 130 and the electrode layer 110, respectively, as in the prior art. The reaction layer 106 can be easily formed, and each of the enzyme layer 106b and the mediator layer 106c contains a hydrophilic polymer that does not have a double bond of an oxygen atom. And the reduction of the mediator of the mediator layer 106c is suppressed, so that the biosensor 100 that can be stored for a long period of time can be easily manufactured.

Description

  The present invention includes an electrode layer provided with an electrode system including a working electrode and a counter electrode, a spacer layer in which a slit for forming a cavity is formed and stacked on the electrode layer, and an air hole communicating with the cavity. The present invention relates to a biosensor manufacturing method including a cover layer laminated on a spacer layer and a reaction layer provided on a working electrode and a counter electrode.

  As shown in the conventional biosensor of FIG. 10, an electrode system including a working electrode 501 and a counter electrode (not shown) and a reference electrode 502, an enzyme layer 503a including an enzyme that specifically reacts with a measurement target substance, and a mediator are provided. Using a biosensor 500 having a reaction layer composed of a mediator layer 503b including a voltage between a working electrode 501 and a counter electrode, a reducing substance generated by a reaction between a measurement target substance contained in a sample and the reaction layer There is known a method for measuring a substance that quantifies a substance to be measured by measuring an oxidation current obtained by oxidization by applying (see, for example, Patent Document 1).

  A biosensor 500 shown in FIG. 10 includes an electrode layer 504 formed by providing an electrode on an insulating substrate such as polyethylene terephthalate or polyimide, and an insulator for preventing a short circuit between the electrodes provided on the electrode layer. A layer 505 and a cover layer 506 are stacked. The electrode layer 504 is provided with a mediator layer 503b, the cover layer 506 is provided with an enzyme layer 503a, and the electrode layer 504 and the cover layer 506 are connected to each other by an adhesive layer 508 made of double-sided tape provided on each of them. By being pasted together, the enzyme layer 503a and the mediator layer 503b are separated and arranged apart from each other.

  The electrode layer 504 is provided with a working electrode 501 and a counter electrode, and a reference electrode 502, and an electrode system is formed in the electrode layer 504 by providing electrode patterns electrically connected to the electrodes 501 and 502, respectively. ing.

  When a liquid sample is supplied into the space where the enzyme layer 503a and the mediator layer 503b face each other, the supplied sample comes into contact with the electrodes 501, 502 and the reaction layer, and the reaction layer dissolves in the sample. .

  The enzyme layer 503a provided on the cover layer 506 contains glucose oxidase and a hydrophilic polymer that specifically react with glucose contained in the sample. The mediator layer 503b provided on the working electrode 501 and the counter electrode contains potassium ferricyanide as a mediator (electron acceptor) and a hydrophilic polymer. The layers 503a and 503b are prevented from being peeled off by the hydrophilic polymer contained in each of the enzyme layer 503a and the mediator layer 503b.

  In addition, ferricyanide ions produced by the dissolution of potassium ferricyanide in the sample are reduced to ferrocyanide ions, which are reductants, by electrons released when glucose is oxidized to gluconolactone by reacting with glucose oxidase. The Therefore, when a sample containing glucose is supplied to the biosensor 500, ferricyanide ions are reduced by electrons released by the oxidation of glucose, and thus glucose contained in the sample and oxidized by an enzymatic reaction. Ferrocyanide ion, which is a reduced form of ferricyanide ion, is generated in an amount corresponding to the concentration of.

  In the biosensor 500 configured as described above, the oxidation current obtained by oxidizing the reduced form of the mediator resulting from the enzyme reaction on the working electrode 501 has a magnitude depending on the glucose concentration in the sample. By measuring the current, glucose contained in the sample can be quantified.

Japanese Unexamined Patent Application Publication No. 2009-244012 (paragraphs 0016 to 0092, FIGS. 1 and 2, abstract, etc.)

  By the way, the enzyme contained in the enzyme layer 503a and the mediator contained in the mediator layer 503b react in the storage state of the biosensor 500, so that the mediator is reduced over time. There is a risk that the measurement accuracy of this will deteriorate. Therefore, in the above-described biosensor 500, the enzyme layer 503a and the mediator layer 503b forming the reaction layer are separated and arranged in a separated state, thereby preventing the reduction of the mediator by the enzyme. However, with this configuration, it is possible to prevent the reaction layer from deteriorating due to the reaction of the enzyme and the mediator due to the biosensor 500 being stored for a long period of time. The layer 503b and the enzyme layer 503a have to be formed, which takes time and increases the manufacturing cost.

  The hydrophilic polymer contained in each of the enzyme layer 503a and the mediator layer 503b prevents the separation of the layers 503a and 503b, or filters the blood sample when the blood sample is supplied to the biosensor 500, for example. By inhibiting the movement of blood cells, it has a function of suppressing the influence of the hematocrit value of the blood sample on the measurement. On the other hand, it is known that the hydrophilic polymer reduces the mediator contained in the mediator layer 503b. For example, when the biosensor 500 is stored for a long period of time, the reduction of the mediator by the hydrophilic polymer proceeds gradually, and when the above-described oxidation current is measured, the reduced form of the mediator that has been reduced by the hydrophilic polymer is oxidized. Since the oxidation current caused by the measurement is also measured as the background current together with the oxidation current to be measured, the measurement accuracy deteriorates.

  Therefore, conventionally, the biosensor 500 is provided with an expiration date, and the biosensor 500 that has been stored for a long time after the expiration date is discarded because the measurement accuracy deteriorates. In the measurement of the measurement target substance contained in the sample, The running cost was increased. As described above, conventionally, sufficient studies have not been made on the influence of hydrophilic polymers on mediators.

  The present invention has been made in view of the above problems, and each of the enzyme layer and the mediator layer includes a hydrophilic polymer that does not have a double bond of an oxygen atom. It aims at providing the technique which can be manufactured in this.

  In order to achieve the above-described object, the biosensor of the present invention includes an electrode layer provided with an electrode system including a working electrode and a counter electrode on one surface of an insulating substrate, a slit, and the slit serving as the function. A spacer layer disposed on the tip side of the electrode and the counter electrode and stacked on the one surface of the electrode layer; a cavity formed by the electrode layer and the slit and supplied with a sample; and air communicating with the cavity A biosensor manufacturing method comprising: a cover layer in which a hole is formed to cover the cavity and stacked on the spacer layer; and a reaction layer provided on a tip side of the working electrode and the counter electrode exposed to the cavity An enzyme layer forming step of forming an enzyme layer containing an enzyme that reacts with a substance to be measured and a hydrophilic polymer that does not have a double bond of an oxygen atom; It is characterized in that it comprises a reaction layer formation step and a mediator layer forming step of forming a mediator layer containing data and a hydrophilic polymer having no double bond oxygen atom (claim 1).

  In the invention configured as described above, the reaction layer provided on the tip side of the working electrode and the counter electrode exposed to the cavity formed by the slit of the spacer layer has a double bond between the enzyme that reacts with the measurement target substance and oxygen atoms. An enzyme layer forming step for forming an enzyme layer containing a hydrophilic polymer that does not have, and a mediator layer forming step for forming a mediator layer containing a mediator and a hydrophilic polymer that does not have a double bond of an oxygen atom It is formed by the reaction layer forming step. Therefore, since the enzyme layer and the mediator layer are formed together as a reaction layer on the tip side of the working electrode and the counter electrode provided in the electrode layer, the enzyme layer and the mediator layer are respectively formed on the cover layer and the electrode layer as in the conventional case. It is not necessary to form each individually, and a reaction layer can be formed easily.

  In addition, an enzyme layer containing an enzyme and a hydrophilic polymer having no oxygen atom double bond, and a mediator and a mediator layer containing a hydrophilic polymer having no oxygen atom double bond are formed. Makes it possible to surround the enzyme contained in the enzyme layer and the mediator contained in the mediator layer with a hydrophilic polymer that does not have a double bond of oxygen atoms, and to form a reaction layer with oxygen and mediator separated. Is done. As a result of intensive studies by the inventor of the present application, when the hydrophilic polymer has an oxygen atom double bond, the mediator is reduced by the nucleophilic attack of the functional group having the oxygen bond double bond against the mediator. Therefore, with this configuration, the enzyme and mediator are surrounded by a hydrophilic polymer that does not have a double bond of oxygen atoms. The mediator and the enzyme contained can be prevented from coming into contact with each other, and the mediator can be prevented from being reduced by the hydrophilic polymer.

  Therefore, a biosensor that can be stored for a long period of time can be easily manufactured by employing this reagent structure.

  Further, the mediator layer is formed after the enzyme layer is formed, and the enzyme layer is disposed at a position closer to the electrode layer. Since the enzyme has a lower diffusion rate than the mediator, the amount of enzyme / mediator in the vicinity of the electrode is larger than when the enzyme is laminated on the mediator, and the responsiveness and measurement accuracy of the sensor are improved.

  The reaction layer forming step is a first intermediate including a hydrophilic polymer having no oxygen atom double bond, which is performed after the enzyme layer forming step and before the mediator layer forming step. It is good to further have the 1st intermediate | middle layer formation process which forms a layer (Claim 2).

  With this configuration, the first intermediate layer containing a hydrophilic polymer having no oxygen atom double bond is formed between the enzyme layer and the mediator layer by the first intermediate layer forming step. Since the first intermediate layer prevents the enzyme contained in the layer from coming into contact with the mediator contained in the mediator layer, it further suppresses the reaction between the enzyme contained in the enzyme layer and the mediator contained in the mediator layer. Can do.

  The reaction layer forming step further includes a hydrophilic layer forming step of forming a hydrophilic layer including a hydrophilic polymer having a double bond of an oxygen atom, which is performed before the enzyme layer forming step. (Claim 3).

  With this configuration, before the enzyme layer is formed, a hydrophilic layer containing a hydrophilic polymer having a double bond of oxygen atoms is formed by the hydrophilic layer forming step. A hydrophilic polymer having a heavy bond has a higher effect of blocking the movement of blood cells and the like than a hydrophilic polymer having no oxygen atom double bond. Therefore, since the hydrophilic layer provided in the electrode layer contains a hydrophilic polymer having a double bond of oxygen atoms, for example, when a blood sample is supplied to the cavity of the biosensor, the hydrophilic layer Since the blood sample is efficiently filtered by the hydrophilic polymer and movement of blood cells contained in the blood sample is prevented, the influence on the measurement accuracy due to the difference in the hematocrit value of the blood sample can be reduced. Therefore, an accurate and highly reliable biosensor can be provided.

  The reaction layer forming step is a second intermediate including a hydrophilic polymer having no oxygen atom double bond, which is performed after the hydrophilic layer forming step and before the enzyme layer forming step. It is good to further have the 2nd intermediate | middle layer formation process which forms a layer (Claim 4).

  If comprised in this way, since the 2nd intermediate | middle layer containing the hydrophilic polymer which does not have the double bond of an oxygen atom is formed by a 2nd intermediate | middle layer formation process between a hydrophilic layer and an enzyme layer, Since the second intermediate layer prevents the hydrophilic polymer having a double bond of oxygen atoms contained in the layer from contacting the mediator contained in the mediator layer, the mediator contained in the mediator layer is hydrophilic in the hydrophilic layer. Reduction by the polymer can be further suppressed.

  The hydrophilic polymer having no oxygen atom double bond includes at least one of hydroxypropylmethylcellulose, hydroxypropylcellulose, methylcellulose, hydroxyethylcellulose, hydroxyethylmethylcellulose, polyvinyl alcohol, and polyethylene glycol. Good (Claim 5).

  When configured in this way, at least one of hydroxypropylmethylcellulose, hydroxypropylcellulose, methylcellulose, hydroxyethylcellulose, hydroxyethylmethylcellulose, polyvinyl alcohol, and polyethylene glycol is a reagent as a hydrophilic polymer having no oxygen atom double bond. By being contained in the layer, the mediator contained in the reagent layer can be prevented from being reduced, and the reagent layer can be prevented from peeling off from the hydrophilic layer. Can be provided.

  The hydrophilic polymer having a double bond of oxygen atoms may contain at least carboxymethylcellulose.

  If comprised in this way, it will prevent that the reagent layer laminated | stacked on a hydrophilic layer peels by providing the hydrophilic layer which contains at least carboxymethylcellulose as a hydrophilic polymer which has a double bond of an oxygen atom on an electrode layer. be able to. In addition, for example, when a blood sample is supplied to the cavity of the biosensor, the blood sample is filtered by the hydrophilic polymer of the hydrophilic layer and the movement of blood cells contained in the blood sample is prevented, so the hematocrit value of the blood sample It is possible to reduce the influence on the measurement accuracy due to the difference.

  According to the present invention, the enzyme layer and the mediator layer are formed together as the reaction layer on the tip side of the working electrode and the counter electrode provided in the electrode layer. It is not necessary to form a layer and a mediator layer separately, a reaction layer can be formed easily, and each of the enzyme layer and the mediator layer contains a hydrophilic polymer having no oxygen atom double bond. In the storage state, the contact between the enzyme contained in the enzyme layer and the mediator contained in the mediator layer is suppressed, and the reduction of the mediator in the mediator layer is suppressed. Can be manufactured.

It is a figure which shows the biosensor concerning 1st Embodiment of this invention, Comprising: (a) is a disassembled perspective view, (b) is a perspective view. It is a cross-sectional view of the cavity part of the biosensor of FIG. It is a figure which shows the manufacturing method of the biosensor concerning 1st Embodiment of this invention, Comprising: (a), (b) shows a different process, respectively. It is a figure which shows the relationship between the storage period of a biosensor, and a background electric current. It is a cross-sectional view of the cavity part of the biosensor according to the second embodiment of the present invention. It is a cross-sectional view of the cavity part of the biosensor according to the third embodiment of the present invention. It is a cross-sectional view of the cavity part of the modification of a biosensor. It is a cross-sectional view of the cavity part of the biosensor according to the fourth embodiment of the present invention. It is a cross-sectional view of the cavity part of the modification of a biosensor. It is a figure which shows the conventional biosensor.

<First Embodiment>
A biosensor according to a first embodiment of the present invention and a method for manufacturing the biosensor will be described with reference to FIGS.

(Configuration and manufacturing method of biosensor)
1A and 1B show a biosensor according to a first embodiment of the present invention, in which FIG. 1A is an exploded perspective view and FIG. 1B is a perspective view. FIG. 2 is a cross-sectional view of the cavity portion of the biosensor of FIG. FIG. 3 is a diagram showing a method for manufacturing the biosensor according to the first embodiment of the present invention, wherein (a) and (b) show different steps.

  The biosensor 100 of the present invention includes an electrode system including a working electrode 101 and a counter electrode 102, and a reaction layer 106 including an enzyme that reacts with a mediator and a substance to be measured, and is used by being attached to a measuring instrument (not shown). It is what is done. That is, a substance to be measured such as glucose contained in a sample such as blood supplied to a cavity 103 provided on the tip side of the biosensor 100 attached to the measuring instrument, and a reaction layer 106 provided on the biosensor 100. By measuring the oxidation current obtained by applying a voltage between the working electrode 101 and the counter electrode 102 to oxidize the reducing substance produced by the reaction of the reaction, the quantitative determination of the measurement target substance contained in the sample Is done.

  That is, as shown in FIGS. 1 and 2, the biosensor 100 includes a working electrode 101 and a counter electrode 102 formed of an insulating material such as ceramic, glass, plastic, paper, biodegradable material, and polyethylene terephthalate, respectively. An electrode layer 110 provided with an electrode system including a cover layer 130 in which an air hole 105 communicating with the cavity 103 is formed, and a slit 104 for forming the cavity 103 is formed, and the electrode layer 110 and the cover layer 130 are formed. The spacer layer 120 is sandwiched between the two layers, and the spacer layer 120 is formed by being laminated and bonded in a state where the tip side where the sample introduction port 103a is provided is aligned. A reaction layer 106 containing an enzyme that reacts with a measurement target substance such as glucose contained in a sample is provided on the working electrode 101 and the counter electrode 102. Then, the biosensor 100 is attached to the measuring instrument by being inserted and attached to a predetermined insertion port of the measuring instrument from the rear end side.

  In this embodiment, the electrode layer 110 is formed of an insulating substrate made of an insulating material such as polyethylene terephthalate. In addition, a conductive layer made of a noble metal such as platinum, gold, palladium, or a conductive material such as carbon, copper, aluminum, titanium, ITO, or ZnO is formed on one surface of the insulating substrate that forms the electrode layer 110 by screen printing or It is formed by sputtering vapor deposition. Then, the conductive layer formed on one surface of the insulating substrate is subjected to patterning by laser processing or photolithography, so that the working electrode 101 and the counter electrode 102 and the biosensor sensor chip 100 are mounted on the measuring instrument. Then, an electrode system including electrode patterns 101a and 102a that electrically connect each of the working electrode 101 and the counter electrode 102 to the measuring instrument is formed.

  In addition, the working electrode 101 and the counter electrode 102 are arranged so that their respective distal end sides are exposed to the cavity 103. In addition, electrode patterns 101a and 102a on the rear end side of each of the working electrode 101 and the counter electrode 102 are edges of the electrode layer 110 on the opposite side to the sample introduction port 103a, and the electrode layer 110 on which the spacer layer 120 is not stacked. It is formed by extending to the edge.

  Next, the spacer layer 120 is laminated on the electrode layer 110 formed as described above. The spacer layer 120 is formed of a substrate made of an insulating material such as polyethylene terephthalate, and a slit 104 for forming the cavity 103 is formed at substantially the center of the front end edge of the substrate. Then, the slit 104 is disposed on the distal end side of the working electrode 101 and the counter electrode 102, and the spacer layer 120 is partially covered and laminated on one surface of the electrode layer 110, so that the electrode layer 110 and the slit 104 are stacked. A cavity 103 to which a sample is supplied is formed.

  Subsequently, after the cavity 103 formed by stacking the spacer layer 120 on the electrode layer 110 is cleaned with plasma, the reaction layer 106 is formed. As the plasma used in the plasma cleaning process, various plasmas used in metal activation treatment by plasma such as oxygen plasma, nitrogen plasma, and argon plasma can be used. Plasma may be used.

  As shown in FIGS. 3A and 3B, the reaction layer 106 is formed on the tip side of the working electrode 101 and the counter electrode 102 exposed to the cavity 103 before the cover layer 130 is laminated on the spacer layer 120. And a reagent 202 containing a hydrophilic polymer not having a double bond of oxygen atom, and 203 containing a mediator and a hydrophilic polymer not having a double bond of oxygen atom in this order are dropped. It is formed. In addition, a hydrophilic agent such as a surfactant or phospholipid is applied to the inner wall of the cavity 104 in order to smoothly supply a sample such as blood to the cavity 104.

  Specifically, the reaction layer 106 is stacked on the electrode layer 110 and includes an enzyme layer 106b including a hydrophilic polymer that does not have a double bond between an enzyme and an oxygen atom, and the enzyme layer 106b. And a mediator layer 106c containing a hydrophilic polymer having no double bond, and formed by the reaction layer forming process as follows.

  That is, as shown in FIG. 3A, a predetermined amount of a reagent 202 containing methylcellulose as a hydrophilic polymer not having a double bond between an enzyme and an oxygen atom is dropped from the dropping device 200 into the cavity 103 and dried. As a result, the enzyme layer 106b is formed (enzyme layer forming step). Next, as shown in FIG. 3B, a predetermined amount of a reagent 203 containing hydroxypropylmethylcellulose as a hydrophilic polymer not having a double bond of a mediator and an oxygen atom is dropped from the dropping device 200 into the cavity 103. When the mediator layer 106c is formed by drying (the mediator layer forming step), the reaction layer 106 is formed.

  As described above, in this embodiment, the “reaction layer forming step” of the present invention is constituted by the enzyme layer forming step and the mediator layer forming step.

  Examples of enzymes include glucose oxidase, lactate oxidase, cholesterol oxidase, alcohol oxidase, sarcosine oxidase, fructosylamine oxidase, pyruvate oxidase, glucose dehydrogenase, lactate dehydrogenase, alcohol dehydrogenase, hydroxybutyrate dehydrogenase, cholesterol esterase, creatininase , Creatinase, DNA polymerase, etc. can be used, and these enzymes can be selected according to the measurement target substance (glucose, lactic acid, cholesterol, alcohol, sarcosine, fructosylamine, pyruvic acid, hydroxybutyric acid, etc.) to be detected. Various sensors can be formed.

  For example, glucose oxidase or glucose dehydrogenase can be used to form a glucose sensor that detects glucose in a blood sample, and alcohol oxidase or alcohol dehydrogenase can be used to form an alcohol sensor that detects ethanol in a blood sample. For example, a lactic acid sensor for detecting lactic acid in a blood sample can be formed, and a total cholesterol sensor can be formed by using a mixture of cholesterol esterase and cholesterol oxidase.

  As the mediator, potassium ferricyanide, ferrocene, ferrocene derivatives, benzoquinone, quinone derivatives, osmium complexes, ruthenium complexes, and the like can be used.

  Further, as the hydrophilic polymer having no oxygen atom double bond, hydroxypropylmethylcellulose, hydroxypropylcellulose, methylcellulose, hydroxyethylcellulose, hydroxyethylmethylcellulose, polyvinyl alcohol, polyethylene glycol, or the like can be used. In addition, the hydrophilic polymer which does not have the double bond of the oxygen atom mixed with the enzyme and the mediator in each of the reagents 202 and 203 functions as a thickener. Two or more hydrophilic polymers having no oxygen atom double bond may be used in combination.

  Moreover, as hydrophilizing agents, surfactants such as Triton X100 (manufactured by Sigma Aldrich), Tween 20 (manufactured by Tokyo Chemical Industry Co., Ltd.), sodium bis (2-ethylhexyl) sulfosuccinate, and phospholipids such as lecithin can be used. . In addition to applying the hydrophilizing agent to the cavity 104 as described above, the hydrophilizing agent may be mixed with each of the reagents 202 and 203 and dropped into the cavity 104, or may be dropped into the cavity 104 after the reagent layer is formed. . Further, a buffering agent such as phosphoric acid may be provided in order to reduce variation in the concentration of ions contained in the sample.

  Next, after the reaction layer 106 is formed in the cavity 103, the cover layer 130 formed of a substrate made of an insulating material such as polyethylene terephthalate is laminated on the spacer layer 120, whereby the biosensor 100 is formed. The As shown in FIGS. 1A and 1B, the cover layer 130 has an air hole 105 that communicates with the cavity 103 when laminated on the spacer layer 120, and the cover layer 130 has the cavity 103. And is laminated on the spacer layer 120.

  In this embodiment, the biosensor 100 is formed for the purpose of quantifying glucose in blood, and FAD (flavin adenine dinucleotide) is used as an enzyme that specifically reacts with glucose as a measurement target substance. Is a mediator that is reduced by electrons generated by the reaction between glucose and FAD-GDH, which is a measurement object, and becomes a reducing substance, including GDH (glucose dehydrogenase) (hereinafter referred to as FAD-GDH). The reaction layer 106 containing potassium ferricyanide is provided on the tip side of the working electrode 101 and the counter electrode 102 exposed to the cavity 103.

  In the biosensor 100 configured as described above, a sample made of blood is brought into contact with the sample introduction port 103a at the tip, whereby the sample is sucked toward the air hole 105 by a capillary phenomenon and supplied to the cavity 103. . Then, when the reaction layer 106 is dissolved in the sample supplied to the cavity 103, electrons are released by an enzyme reaction between glucose as a measurement target substance in the sample and FAD-GDH, and ferricyanization is performed by the emitted electrons. The ions are reduced to produce ferrocyanide ions, which are reducing substances. Then, a voltage (for example, 0.3 V) is applied between the working electrode 101 and the counter electrode 102 of the biosensor 100 with respect to the reducing substance generated by the oxidation-reduction reaction caused by the reaction layer 106 dissolving in the sample. The glucose in the sample is quantified in the measuring instrument by measuring the oxidation current flowing between the working electrode 101 and the counter electrode 102 by oxidation. In addition, after a voltage is applied between the working electrode 101 and the counter electrode 102 of the biosensor 100, a current value after 3 to 5 seconds is measured as an oxidation current.

(Background current comparison example)
FIG. 4 is a diagram illustrating the relationship between the storage period of the biosensor and the background current, where the horizontal axis indicates the storage period (h), and the vertical axis indicates the magnitude of the background current (μA). Also, ◆ in the figure indicates the background current of a conventional biosensor in which the enzyme layer 106b and the mediator layer 106c do not contain a hydrophilic polymer having no oxygen atom double bond, Indicates the background current of the biosensor 100 of the present embodiment. The background current was measured by supplying a sample for measuring the background current to the cavity 103 and then measuring the oxidation current in the same manner as in a normal procedure.

  As shown in FIG. 4, the background current increases with time in the conventional biosensor as the storage period of the biosensor increases, whereas in the biosensor 100 of the present embodiment, the background current increases. The increase is suppressed.

  As described above, according to this embodiment, the working electrode 101 exposed to the cavity 103 formed by the slit 104 of the spacer layer 120 and the reaction layer 106 provided on the distal end side of the counter electrode 102 are glucose that is a measurement target substance. An enzyme layer forming step for forming an enzyme layer 106b containing methylcellulose that does not have an oxygen atom double bond and an enzyme that reacts with oxygen, and a mediator layer that contains a mediator and hydroxypropyl methylcellulose that does not have an oxygen atom double bond It forms by the reaction layer formation process which has the mediator layer formation process to form. Therefore, the enzyme layer 106b and the mediator layer 106c are formed together as the reaction layer 106 on the tip side of the working electrode 101 and the counter electrode 102 provided on the electrode layer 110, so that the cover layer 130 and the electrode layer 110 are conventionally formed. There is no need to form the enzyme layer 106b and the mediator layer 106c respectively, and the reaction layer 106 can be formed easily.

  In addition, an enzyme layer 106b including a hydrophilic polymer having no enzyme and oxygen atom double bond, and a mediator layer 106c including a mediator and a hydrophilic polymer having no oxygen atom double bond are formed. As a result, the enzyme included in the enzyme layer 106b and the mediator included in the mediator layer 106c are surrounded by a hydrophilic polymer that does not have a double bond of oxygen atoms, and the oxygen and the mediator are separated. A reaction layer 106 is formed. As a result of intensive studies by the inventor of the present application, when the hydrophilic polymer has an oxygen atom double bond, the mediator is reduced by the nucleophilic attack of the functional group having the oxygen bond double bond against the mediator. Therefore, with this configuration, the enzyme and the mediator are surrounded by a hydrophilic polymer that does not have a double bond of oxygen atoms. The mediator and enzyme contained in 106 can be prevented from contacting each other, and the mediator can be prevented from being reduced by the hydrophilic polymer.

  Therefore, each of the enzyme layer 106b and the mediator layer 106c contains a hydrophilic polymer that does not have an oxygen atom double bond, so that the enzyme contained in the enzyme layer 106b reacts with the mediator contained in the mediator layer 106c in the storage state. And the reduction of the mediator of the mediator layer 106c is suppressed, so that a biosensor that can be stored for a long period of time can be easily manufactured.

  In addition, the mediator layer 106c is formed after the enzyme layer 106b is formed, and the enzyme layer 106b is disposed at a position closer to the electrode layer 1110. Therefore, the mediator dissolved in the sample supplied to the cavity 103 is not electrode layer. When diffusing toward the electrode 110, as a result of the enzyme reaction, the substance to be measured such as glucose in the sample is oxidized and passes through the enzyme layer 106b rich in electrons. This is practical because the mediator that diffuses toward the surface is efficiently reduced.

  Further, at least one of hydroxypropylmethylcellulose, hydroxypropylcellulose, methylcellulose, hydroxyethylcellulose, hydroxyethylmethylcellulose, polyvinyl alcohol, and polyethylene glycol is included in the reagent layer as a hydrophilic polymer having no oxygen atom double bond. Thus, the mediator contained in the reagent layer can be prevented from being reduced, and the reagent layer can be prevented from peeling off from the electrode layer 110 or the hydrophilic layer 106a. A sensor 110 can be provided.

Second Embodiment
A biosensor manufacturing method according to a second embodiment of the present invention will be described with reference to FIG. FIG. 5 is a cross-sectional view of the cavity portion of the biosensor according to the second embodiment of the present invention. As shown in FIG. 5, this embodiment differs from the first embodiment described above in the first intermediate layer forming step performed after the enzyme layer forming step and before the mediator layer forming step. When a predetermined amount of a reagent containing a hydrophilic polymer having no double bond is dropped into the cavity 103 and dried, the enzyme layer 106b and the mediator layer 106c have a double bond of oxygen atoms. An intermediate layer 106d (first intermediate layer) containing no hydrophilic polymer is further formed. Since the other configuration is the same as that of the first embodiment described above, the description of the configuration and operation is omitted by attaching the same reference numerals.

  With this configuration, since the intermediate layer 106d containing a hydrophilic polymer having no oxygen atom double bond is formed between the enzyme layer 106b and the mediator layer 106c by the first intermediate layer forming step, Since the intermediate layer 106d prevents the enzyme contained in the enzyme layer 106b from contacting the mediator contained in the mediator layer 106c, the enzyme contained in the enzyme layer 106b reacts with the mediator contained in the mediator layer 106c. Further suppression can be achieved.

<Third Embodiment>
A biosensor manufacturing method according to a third embodiment of the present invention will be described with reference to FIG. FIG. 6 is a cross-sectional view of the cavity portion of the biosensor according to the third embodiment of the present invention. As shown in FIG. 6, this embodiment differs from the first embodiment described above as a hydrophilic polymer having a double bond of oxygen atoms in the hydrophilic layer forming step performed before the enzyme layer forming step. A predetermined amount of a reagent containing carboxymethylcellulose (CMC) is dropped into the cavity 103 and dried, whereby the hydrophilic layer 106a is formed on the electrode layer 110 before the enzyme layer 106b is formed. Since the other configuration is the same as that of the first embodiment described above, the description of the configuration and operation is omitted by attaching the same reference numerals.

  With this configuration, before the enzyme layer 106b is formed, the hydrophilic layer 106a containing a hydrophilic polymer (CMC) having a double bond of oxygen atoms is formed by the hydrophilic layer forming step. The hydrophilic polymer having a double bond of oxygen atom has a higher effect of blocking the movement of blood cells and the like than the hydrophilic polymer having no double bond of oxygen atom. Accordingly, since the hydrophilic layer 106a provided in the electrode layer 110 contains a hydrophilic polymer having a double bond of oxygen atoms, for example, when a blood sample is supplied to the cavity 103 of the biosensor 100, Since the blood sample is efficiently filtered by the hydrophilic polymer of the hydrophilic layer 106a and the movement of blood cells contained in the blood sample is prevented, the influence on the measurement accuracy due to the difference in the hematocrit value of the blood sample is reduced. Can do.

  Therefore, an accurate and highly reliable biosensor 100 can be provided. In addition, by providing the hydrophilic layer 106a containing a hydrophilic polymer having a double bond of an oxygen atom on the electrode layer 110, the enzyme layer 106b stacked on the hydrophilic layer 106a can be prevented from peeling off.

  The hydrophilic polymer having a double bond of oxygen atom includes carbonyl group, acyl group, carboxyl group, aldehyde group, sulfo group, sulfonyl group, sulfoxide group, tosyl group, nitro group, nitroso group, ester group, keto group. A polymer having a group, a ketene group, or the like can be used. Two or more hydrophilic polymers having a double bond of an oxygen atom may be used in combination.

  Moreover, as shown in the cross-sectional view of the cavity portion of the modified example of the biosensor of FIG. 7, in the biosensor 100 of FIG. 5, before the enzyme layer 106b is formed, the hydrophilic layer 106a is formed into the electrode layer by the hydrophilic layer forming step. 110 may be formed. Even if it comprises in this way, there can exist the same effect.

<Fourth embodiment>
A biosensor manufacturing method according to the fourth embodiment of the present invention will be described with reference to FIG. FIG. 8 is a cross-sectional view of the cavity portion of the biosensor according to the fourth embodiment of the present invention. As shown in FIG. 8, this embodiment differs from the third embodiment described above in the second intermediate layer forming step performed after the hydrophilic layer forming step and before the enzyme layer forming step. When a predetermined amount of a reagent containing a hydrophilic polymer having no double bond is dropped into the cavity 103 and dried, oxygen atoms have a double bond between the hydrophilic layer 106a and the enzyme layer 106b. An intermediate layer 106d (second intermediate layer) containing no hydrophilic polymer is further formed. Since the other configuration is the same as that of the first embodiment described above, the description of the configuration and operation is omitted by attaching the same reference numerals.

  With this configuration, the intermediate layer 106d containing a hydrophilic polymer having no oxygen atom double bond is formed between the hydrophilic layer 106a and the enzyme layer 106b by the second intermediate layer forming step. Since the intermediate layer 106d prevents the hydrophilic polymer having a double bond of oxygen atoms contained in the hydrophilic layer 106a from coming into contact with the mediator contained in the mediator layer 106c, the mediator contained in the mediator layer 106c becomes a hydrophilic layer. Reduction by the hydrophilic polymer 106a can be suppressed.

  Further, as shown in the cross-sectional view of the cavity portion of the modification of the biosensor of FIG. 9, in the biosensor 100 of FIG. 7, the hydrophilic layer 106a is formed by the second intermediate layer forming step before the enzyme layer 106b is formed. An intermediate layer 106d may be formed thereon. Even if it comprises in this way, there can exist the same effect.

  The present invention is not limited to the above-described embodiment, and various modifications other than those described above can be made without departing from the spirit thereof, for example, a double bond of an oxygen atom can be made. Properly mixing and mixing multiple types of hydrophilic polymers that do not have, effectively block the movement of blood cells in the blood sample, reduce the diffusion and mixing of the enzyme layer and mediator layer, reduce the mediator An inhibitory effect of suppressing reduction can be achieved.

  Further, an ethanol sensor, a lactic acid sensor, or the like may be formed by changing the combination of the enzyme and the mediator included in the reaction layer 106 of the biosensor 100 described above.

  In the above-described embodiment, the biosensor 100 is formed in a bipolar electrode structure having the working electrode 101 and the counter electrode 102. However, the biosensor 100 is formed in a tripolar electrode structure by further providing a reference electrode. May be. In this case, a predetermined potential based on the counter electrode 102 may be applied to the working electrode 101 in a state where the counter electrode 102 is grounded and a reference potential is applied to the reference electrode by the voltage output unit.

  In the above-described embodiment, a blood sample is placed in the cavity 103 by monitoring a current flowing between the working electrode 101 and the counter electrode 102 by applying a predetermined voltage between the working electrode 101 and the counter electrode 102. Although it is detected that the sample has been supplied, a detection electrode for detecting that the sample has been supplied to the cavity 103 may be further provided. In this case, by applying a predetermined voltage between the counter electrode 102 and the detection electrode, the current flowing between the counter electrode 102 and the detection electrode is monitored to detect that the sample is supplied to the cavity 103. do it.

  In addition, of the electrode layer 110, the spacer layer 120, and the cover layer 130 that form the biosensor 100, at least the cover layer 130 is formed of a transparent member so that it can be visually confirmed that the blood sample has been supplied to the cavity 103. Is desirable.

  An electrode layer provided with an electrode system including a working electrode and a counter electrode, a spacer layer in which slits for forming a cavity are formed and stacked on the electrode layer, and an air hole communicating with the cavity are formed in the spacer layer. The present invention can be widely applied to biosensors including a laminated cover layer and reaction layers provided on the working electrode and the counter electrode.

DESCRIPTION OF SYMBOLS 100 Biosensor 101 Working electrode 102 Counter electrode 103 Cavity 104 Slit 105 Air hole 106 Reaction layer 106a Hydrophilic layer 106b Enzyme layer 106c Mediator layer 106d Intermediate layer (1st intermediate layer, 2nd intermediate layer)
110 Electrode layer 120 Spacer layer 130 Cover layer

The present invention includes an electrode layer provided with an electrode system including a working electrode and a counter electrode, a spacer layer in which a slit for forming a cavity is formed and stacked on the electrode layer, and an air hole communicating with the cavity. a cover layer which is laminated on the spacer layer Te, and a reaction layer provided on the working electrode and the counter electrode, a method for manufacturing a biosensor and its.

The present invention has been made in view of the above problems by including a hydrophilic polymer, each enzyme layer and mediator layer does not have a double bond oxygen atom, long-term storable biosensor, and It aims at providing the technique which can manufacture the said biosensor easily.

In order to achieve the above-described object, according to the first aspect of the present invention, an electrode layer provided with an electrode system including a working electrode and a counter electrode is formed on one surface of an insulating substrate, and a slit is formed. A spacer layer disposed on the front side of the working electrode and the counter electrode and stacked on the one surface of the electrode layer, a cavity formed by the electrode layer and the slit and supplied with a sample, and communicated with the cavity Production of a biosensor comprising a cover layer that is formed with an air hole so as to cover the cavity and is laminated on the spacer layer, and a reaction layer provided on the tip side of the working electrode and the counter electrode exposed to the cavity a method, an enzyme layer forming step of forming an enzyme layer comprising a hydrophilic polymer having no double bonds of the enzyme and oxygen atoms that react with the analyte, mediator Comprising a reaction layer formation step and a mediator layer forming step of forming a mediator layer containing a hydrophilic polymer having no double bond oxygen atom and, before Symbol reaction layer forming step, the enzyme layer forming step It is performed before, and further comprising a hydrophilic layer formation step of forming a hydrophilic layer containing a hydrophilic polymer that have a double bond oxygen atom (claim 1).

Furthermore, the reaction layer forming step further includes a hydrophilic layer forming step of forming a hydrophilic layer including a hydrophilic polymer having a double bond of oxygen atoms, which is performed before the enzyme layer forming step . . Therefore, before the enzyme layer is formed, a hydrophilic layer containing a hydrophilic polymer having a double bond of oxygen atoms is formed by a hydrophilic layer forming step. parent aqueous polymer having the effect higher prevent the movement of the blood cells than the hydrophilic polymer that has no double bond oxygen atom. Accordingly, the hydrophilic layer provided on the electrode layer, for that having a double bond oxygen atoms hydrophilic polymer is included, for example, when a blood sample into the cavity of the biosensor is supplied, hydrophilic since the blood sample with a hydrophilic polymer layer move contains Murrell blood cells is inhibited is efficiently filtered blood sample, it is possible to reduce the influence on the measurement accuracy caused by the difference in the hematocrit value of the blood sample . Therefore, an accurate and highly reliable biosensor can be provided .
The reaction layer forming step is a first intermediate including a hydrophilic polymer having no oxygen atom double bond, which is performed after the enzyme layer forming step and before the mediator layer forming step. It is good to further have the 1st intermediate | middle layer formation process which forms a layer (Claim 2).

The reaction layer forming step is a second intermediate including a hydrophilic polymer having no oxygen atom double bond, which is performed after the hydrophilic layer forming step and before the enzyme layer forming step. It is good to further have the 2nd intermediate | middle layer formation process which forms a layer (Claim 3 ).

If comprised in this way, since the 2nd intermediate | middle layer containing the hydrophilic polymer which does not have the double bond of an oxygen atom is formed by a 2nd intermediate | middle layer formation process between a hydrophilic layer and an enzyme layer, Since the second intermediate layer prevents the hydrophilic polymer having a double bond of oxygen atoms contained in the layer from contacting the mediator contained in the mediator layer, the mediator contained in the mediator layer is hydrophilic in the hydrophilic layer. Reduction by the polymer can be further suppressed.
In order to achieve the above object, a second aspect of the present invention, an insulating electrode layer electrode system is provided including a work for electrode and a counter electrode on one surface of the substrate, the slit is formed, the a spacer layer slit bets is Ru is laminated on the one surface of the electrode layer is disposed on the distal side of the working electrode and the counter electrode, and a calibration activity which the sample is supplied is formed by the electrode layer and the slit, a cover layer which is laminated on the spacer layer covers the cavity air hole is formed which communicates with the cavity, and a reaction layer wherein provided at the distal end of the working electrode and the counter electrode is exposed to the cavity a method of manufacturing a biosensor and a enzyme layer forming step of forming an enzyme layer comprising a hydrophilic polymer having no double bonds of the enzyme and oxygen atoms that react with the measurement target substances, media E Bei reaction layer formation step and a mediator layer forming step of forming a mediator layer containing a hydrophilic polymer having no double bonds over data and oxygen atoms, said reaction layer formation step, the enzyme layer formed The method further includes a reduction suppression layer forming step for forming a reduction suppression layer including a hydrophilic polymer having no oxygen atom double bond, which is performed before the step .

If comprised in this way, it will prevent that the reagent layer laminated | stacked on a hydrophilic layer peels by providing the hydrophilic layer which contains at least carboxymethylcellulose as a hydrophilic polymer which has a double bond of an oxygen atom on an electrode layer. be able to. In addition, for example, when a blood sample is supplied to the cavity of the biosensor, the blood sample is filtered by the hydrophilic polymer of the hydrophilic layer and the movement of blood cells contained in the blood sample is prevented, so the hematocrit value of the blood sample It is possible to reduce the influence on the measurement accuracy due to the difference.
Furthermore, in order to achieve the above-described object, the third aspect of the present invention includes an electrode layer provided with an electrode system including a working electrode and a counter electrode on one surface of an insulating substrate, and a slit. a spacer layer is laminated on the one surface of the electrode layer Tsu bets is disposed on the distal end side of the working electrode and the counter electrode, and a key Yabiti which is formed the sample supplied by the electrode layer and the slit, a cover layer which is laminated before Symbol spacer layer covers the cavity air hole that communicates is formed in the cavity, and a reaction layer provided on the tip side of the working electrode and the counter electrode is exposed to the cavity a biosensor comprising a, in the reaction layer, the reduction suppressing layer containing a hydrophilic polymer having no double bond oxygen radicals, and enzyme and mediator you react with the analyte, Reagent layer containing a hydrophilic polymer having no double bonds atom is provided, wherein the reagent layer includes an enzyme layer comprising a hydrophilic high molecule that has no double bond of the enzyme and the oxygen atom And a mediator layer containing a hydrophilic polymer not having a double bond of the oxygen atom and the oxygen atom .

If comprised in this way, since the 2nd intermediate | middle layer containing the hydrophilic polymer which does not have the double bond of an oxygen atom is formed by a 2nd intermediate | middle layer formation process between a hydrophilic layer and an enzyme layer, Since the second intermediate layer prevents the hydrophilic polymer having a double bond of oxygen atoms contained in the layer from contacting the mediator contained in the mediator layer, the mediator contained in the mediator layer is hydrophilic in the hydrophilic layer. Reduction by the polymer can be further suppressed.
In order to achieve the above-described object, the second aspect of the present invention includes an electrode layer provided with an electrode system including a working electrode and a counter electrode on one surface of an insulating substrate, and a slit, Is disposed on the tip side of the working electrode and the counter electrode and is laminated on the one surface of the electrode layer, a cavity formed by the electrode layer and the slit and supplied with a sample, and a cavity A biosensor comprising: a cover layer that is formed in a communicating air hole so as to cover the cavity and is stacked on the spacer layer; and a reaction layer provided on a tip side of the working electrode and the counter electrode exposed to the cavity An enzyme layer forming step of forming an enzyme layer containing an enzyme that reacts with a substance to be measured and a hydrophilic polymer that does not have a double bond of an oxygen atom; And a mediator layer forming step of forming a mediator layer including a mediator layer containing a hydrophilic polymer not having a double bond of oxygen atoms and oxygen atoms, wherein the reaction layer forming step includes the enzyme layer forming step of being performed before, it has an oxygen atom double bonds no hydrophilic polymer further reduction inhibiting layer forming step of forming a suppressing reduction suppressing layer reduction of unrealized said mediator (according Item 4) .

If comprised in this way, it will prevent that the reagent layer laminated | stacked on a hydrophilic layer peels by providing the hydrophilic layer which contains at least carboxymethylcellulose as a hydrophilic polymer which has a double bond of an oxygen atom on an electrode layer. be able to. In addition, for example, when a blood sample is supplied to the cavity of the biosensor, the blood sample is filtered by the hydrophilic polymer of the hydrophilic layer and the movement of blood cells contained in the blood sample is prevented, so the hematocrit value of the blood sample It is possible to reduce the influence on the measurement accuracy due to the difference.
Furthermore, in order to achieve the above-described object, the third aspect of the present invention includes an electrode layer provided with an electrode system including a working electrode and a counter electrode on one surface of an insulating substrate, and a slit formed therein. Is disposed on the tip side of the working electrode and the counter electrode and is laminated on the one surface of the electrode layer, a cavity formed by the electrode layer and the slit and supplied with a sample, and a cavity A biosensor comprising: a cover layer that is formed in a communicating air hole so as to cover the cavity and is stacked on the spacer layer; and a reaction layer provided on a tip side of the working electrode and the counter electrode exposed to the cavity a is, in the reaction layer, the hydrophilic polymer that has no double bond oxygen atoms to suppress the reduction suppressing layer reduction of unrealized the mediator analyte and anti And a reagent layer containing a hydrophilic polymer that does not have a double bond of an oxygen atom, and the reagent layer has a high hydrophilicity that does not have a double bond of the enzyme and the oxygen atom. An enzyme layer including a molecule and a mediator layer including a hydrophilic polymer not having a double bond of the mediator and the oxygen atom are provided (claim 7) .

Claims (6)

An electrode layer provided with an electrode system including a working electrode and a counter electrode on one surface of an insulating substrate;
A spacer layer formed on the one surface of the electrode layer, the slit being formed on the tip side of the working electrode and the counter electrode;
A cavity formed by the electrode layer and the slit and supplied with a sample;
An air hole communicating with the cavity to cover the cavity and be laminated on the spacer layer;
In a method for producing a biosensor comprising the working electrode exposed in the cavity and a reaction layer provided on a tip side of the counter electrode,
An enzyme layer forming step of forming an enzyme layer containing an enzyme that reacts with a substance to be measured and a hydrophilic polymer that does not have a double bond of an oxygen atom;
A biosensor manufacturing method comprising: a reaction layer forming step including a mediator layer forming step of forming a mediator layer containing a mediator and a hydrophilic polymer having no oxygen atom double bond.   The reaction layer forming step includes a first intermediate layer including a hydrophilic polymer having no oxygen atom double bond, which is performed after the enzyme layer forming step and before the mediator layer forming step. The biosensor manufacturing method according to claim 1, further comprising a first intermediate layer forming step to be formed.   The reaction layer forming step further includes a hydrophilic layer forming step of forming a hydrophilic layer including a hydrophilic polymer having a double bond of an oxygen atom, which is performed before the enzyme layer forming step. The manufacturing method of the biosensor of Claim 1 or 2.   The reaction layer forming step includes a second intermediate layer including a hydrophilic polymer having no oxygen atom double bond, which is performed after the hydrophilic layer forming step and before the enzyme layer forming step. The biosensor manufacturing method according to claim 3, further comprising a second intermediate layer forming step of forming.   The hydrophilic polymer having no oxygen atom double bond includes at least one of hydroxypropylmethylcellulose, hydroxypropylcellulose, methylcellulose, hydroxyethylcellulose, hydroxyethylmethylcellulose, polyvinyl alcohol, and polyethylene glycol. A method for producing a biosensor according to any one of claims 1 to 4.   The method for producing a biosensor according to any one of claims 1 to 5, wherein the hydrophilic polymer having a double bond of an oxygen atom contains at least carboxymethylcellulose.

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